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β-内酰胺酶在用于检测微生物抗原的酶免疫测定中的应用。

The use of beta-lactamase in enzyme immunoassays for detection of microbial antigens.

作者信息

Yolken R H, Wee S B, Van Regenmortel M

出版信息

J Immunol Methods. 1984 Oct 12;73(1):109-23. doi: 10.1016/0022-1759(84)90036-x.

Abstract

The sensitivity and performance characteristics of enzyme immunoassays (EIA) depend to a great extent on the kinetics of the enzyme-substrate system used as indicator. We labeled a variety of polyclonal and monoclonal immunoglobulins with purified beta-lactamase and used them in sensitive EIA systems for the detection of a number of microbial antigens. Polyclonal antibodies to rotavirus, adenovirus, and Haemophilus influenzae type b polyribitol phosphate and monoclonal antibodies to dengue virus were labeled with beta-lactamase and used to provide sensitive direct EIA systems for the detection of the corresponding antigens. In addition, antibodies directed at animal immunoglobulins were labeled with beta-lactamase and used in indirect EIA for the detection of viral antigens with unlabeled anti-viral monoclonal and polyclonal antibodies. Similarly, avidin from Streptomyces was labeled with beta-lactamase and used to detect viral antigens tested for in an avidin-biotin format. Enzyme immunoassay systems with beta-lactamase-labeled antibodies were also used to detect rotaviral and adenoviral antigens in rectal swab specimens from children with acute gastroenteritis. The sensitivity of the beta-lactamase EIA compared favorably with that of analogous EIA systems using alkaline phosphatase or horseradish peroxidase. The results of a beta-lactamase EIA were easily determined by naked eye and a permanent record of the qualitative results obtained by the use of a standard office photocopier, obviating the need for an expensive colorimeter. Enzyme immunoassays using beta-lactamase have potential as practical assay systems for the detection of a wide range of microbial antigens using monoclonal and polyclonal antibodies.

摘要

酶免疫测定法(EIA)的灵敏度和性能特征在很大程度上取决于用作指示剂的酶 - 底物系统的动力学。我们用纯化的β - 内酰胺酶标记了多种多克隆和单克隆免疫球蛋白,并将它们用于灵敏的EIA系统中,以检测多种微生物抗原。针对轮状病毒、腺病毒和b型流感嗜血杆菌多聚核糖醇磷酸的多克隆抗体以及针对登革病毒的单克隆抗体用β - 内酰胺酶进行了标记,并用于提供灵敏的直接EIA系统,以检测相应的抗原。此外,针对动物免疫球蛋白的抗体用β - 内酰胺酶进行了标记,并用于间接EIA中,以使用未标记的抗病毒单克隆和多克隆抗体检测病毒抗原。同样,来自链霉菌的抗生物素蛋白用β - 内酰胺酶进行了标记,并用于以抗生物素蛋白 - 生物素形式检测所测试的病毒抗原。用β - 内酰胺酶标记抗体的酶免疫测定系统也用于检测急性胃肠炎患儿直肠拭子标本中的轮状病毒和腺病毒抗原。与使用碱性磷酸酶或辣根过氧化物酶的类似EIA系统相比,β - 内酰胺酶EIA的灵敏度更具优势。β - 内酰胺酶EIA的结果通过肉眼即可轻松确定,并且使用标准办公复印机即可获得定性结果的永久记录,无需昂贵的比色计。使用β - 内酰胺酶的酶免疫测定法有潜力成为使用单克隆和多克隆抗体检测多种微生物抗原的实用测定系统。

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